The present invention is directed to compositions and methods to modulate inflammatory and immune responses in a subject, which includes immune activation and inhibiting inflammatory responses, by modulating the regeneration and tolerance factor (RTF).
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1. A method for inducing apoptosis in an ovarian carcinoma cell comprising administering an effective amount of anti-Regeneration and Tolerance Factor (RTF) antibody.
3. A method for treating ovarian carcinoma in a mammalian subject comprising administering an effective amount of anti-Regeneration and Tolerance Factor (RTF) antibody.
2. The method of
4. The method of
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This application claims priority from U.S. Provisional Patent Application No. 60/446,499 which was filed on Feb. 10, 2003.
The inflammatory process initiates a localized defense against foreign antigens. The process is characterized by immune activation as well as destruction of nearby tissues secondary to involved release of destructive agents. Initially involved tissue assumes a significant role in provoking the inflammatory response at large (Matzinger, P., The danger model: a renewed sense of self. Science, 2002. 296(5566): p. 301–5; Medzhitov, R. and C. A. Janeway, Jr., Decoding the patterns of self and nonself by the innate immune system. Science, 2002. 296(5566): p. 298–300). One of the primary immunogenic mechanisms triggered by the inflammatory response includes the release of ATP into the extracellular space. ATP is liberated from injured tissue itself—as well as from nearby macrophages, neutrophils, platelets and dying cells—following incidents of stress, infection or other forms of tissue insult (Fredholm, B. B., Purines and neutrophil leukocytes. Gen Pharmacol, 1997. 28(3): p. 345–50; Beigi, R., et al., Detection of local ATP release from activated platelets using cell surface-attached firefly luciferase. Am J Physiol, 1999. 276(1 Pt 1): p. C267–78; Schwiebert, E. M., ABC transporter-facilitated ATP conductive transport. Am J Physiol, 1999. 276(1 Pt 1): p. C1-8; Mizumoto, N., et al., CD39 is the dominant Langerhans cell-associated ecto-NTPDase: modulatory roles in inflammation and immune responsiveness. Nat Med, 2002. 8(4): p. 358–65; Dubyak, G. R. and C. el-Moatassim, Signal transduction via P2-purinergic receptors for extracellular ATP and other nucleotides. Am J Physiol, 1993. 265(3 Pt 1): p. C577–606; Gordon, J. L., Extracellular ATP: effects, sources and fate. Biochem J, 1986. 233(2): p. 309–19). Extracellular ATP can then exert a wide variety of effects on surrounding cells, most notably the induction of apoptotic events leading ultimately to cell death in both lymphocytes and macrophages (Di Virgilio, F., The P2Z purinoceptor: an intriguing role in immunity, inflammation and cell death. Immunol Today, 1995. 16(11): p. 524–8; Gargett, C. E., J. E. Cornish, and J. S. Wiley, ATP, a partial agonist for the P2Z receptor of human lymphocytes. Br J Pharmacol, 1997. 122(5): p. 911–7; Buisman, H. P., et al., Extracellular ATP induces a large nonselective conductance in macrophage plasma membranes. Proc Natl Acad Sci USA, 1988. 85(21): p. 7988–92; Ferrari, D., et al., ATP-mediated cytotoxicity in microglial cells. Neuropharmacology, 1997. 36(9): p. 1295–301; Zheng, L. M., et al., Extracellular ATP as a trigger for apoptosis or programmed cell death. J Cell Biol, 1991. 112(2): p. 279–88). Diminution of cell integrity then leads to further ATP release, propagating the inflammatory response and continued tissue destruction. Recent data have shown an attenuated effect of extracellular ATP in the presence of the regeneration and tolerance factor (RTF) protein. The present invention discloses compositions and methods to modulate inflammatory and immune responses by regulating the activities of RTF. RTF prevents ATP activation of P2Z, thus preventing the cell from undergoing pro-inflammatory activation and apoptosis.
The present invention is directed to compositions and methods to modulate inflammatory and immune responses in a subject, which includes immune activation and inhibiting inflammatory responses, by modulating the regeneration and tolerance factor (RTF). Immune activation can be accomplished by inhibiting the RTF activity. In one embodiment, the RTF activity can be inhibited by administering a RTF antagonist, which can be a small molecule, a peptide, or an antibody or a fragment thereof. Inhibiting the RTF activity may result in cell apotosis, especially cancer cells such as ovarian carcinoma cells.
Inflammatory responses can be inhibited by increasing the level of activity of RTF. In an embodiment, the method of increasing the level of activity of RTF is by administering an effective amount of RTF or a fragment of RTF. The RTF or its fragment can be isolated or purified from mammalian cells such as the T-lymphocyte, the B-lymphocyte, the macrophage, thymus, or the fetalplacental tissue. Alternatively, the RTF can be synthetic or a recombinant RTF.
The present invention is also directed to a method of treating cancer, such as ovarian cancer, by inhibiting the RTF activity. In one embodiment, the method to inhibit RTF activity is to administer an effective dose of a RTF antagonist.
The present invention is further directed to a method of treating or ameliorating an inflammatory disorder or an autoimmune disorder or one or more symptoms thereof by administering an effective amount of RTF or a fragment of RTF. The RTF or its fragment can be isolated or purified from mammalian cells such as the T-lymphocyte, the B-lymphocyte, the macrophage, thymus, or the fetalplacental tissue. Alternatively, the RTF can be synthetic or a recombinant RTF. The RTF can be formulated with one or more suitable pharmaceutical excipients for administration by parenteral, intramuscular, topical, nasal, pulmonary, or oral route. The formulation can also be in the form of microparticles or nanoparticles. In an embodiment, the method of treating or ameliorating an inflammatory disorder or an autoimmune disorder or one or more symptoms thereof includes an additional step of administering a TNF-α antagonist, which includes but is not limited to infliximab, etanercept, D2E7, CDP571, CDP870, thalidomide and its analogs, and phosphodiesterase type IV inhibitors.
Additional features and advantages of the present invention are described in, and will be apparent from, the following Detailed Description of the Invention and the figures.
The present invention is directed to compositions and methods to modulate inflammatory and immune responses in a subject by regulating the level of activity of regeneration and tolerance factor (RTF). Modulating inflammatory and immune responses includes both immune activation and the inhibition of the inflammatory responses. In a preferred embodiment, the subject is a mammal. In a more preferred embodiment, the subject is a human.
A principle means by which RTF controls the extent of inflammation is via its interaction with P2Z, a cell surface receptor expressed primarily on cells of hematopoetic origin such as lymphocytes and macrophages. P2Z is one of a family of receptors known as purinoceptors which are activated by nucleotides. Extracellular ATP binds P2Z, which triggers the opening of specific calcium channels as well as non-specific transmembrane channels (Dubyak, G. R. and C. el-Moatassim, Signal transduction via P2-purinergic receptors for extracellular ATP and other nucleotides. Am J Physiol, 1993. 265(3 Pt 1): p. C577–606; Gargett, C. E., J. E. Cornish, and J. S. Wiley, ATP, a partial agonist for the P2Z receptor of human lymphocytes. Br J Pharmacol, 1997. 122(5): p. 911–7; Zheng, L. M., et al., Extracellular ATP as a trigger for apoptosis or programmed cell death. J Cell Biol, 1991. 112(2): p. 279–88). These channels then allow for rapid influx of calcium ions into the cytosolic space. This calcium influx in turn drives forward many specific activation pathways. The activation of P2Z can cause specific activation of NF-κB, and the maturation and secretion of IL-1β, a potent inflammatory cytokine. This will subsequently increase both cellular activation and drive the inflammatory response, making P2Z a key mediator in the inflammatory process. It can also cause apoptosis and an inflammatory counterpart to apoptosis, oncosis, inducing the release of further ATP. Recent reports have shown that the absence of the P2Z purinoceptor can attenuate the inflammatory response (Labasi J M, P. N., Donovan C, McCurdy S, Lira P, Payette M M, Brissette W, Wicks J R, Audoly L, Gabel C A., Absence of the P2X7 receptor alters leukocyte function and attenuates an inflammatory response. J Immunol, 2002. 168(12)(Jun 15): p. 6436–45).
Therefore it follows that extracellular ATP up-regulates the inflammatory response through its instigation of P2Z activation at the site of inflammation and also the stimulated release of pro-inflammatory cytokines. A key regulatory point at which to reduce the inflammatory response, then, is in the concentration of extracellular ATP. It has been suggested that ecto-ATPases hold important regulatory surface ATPase activity, which attenuates inflammatory as well as immune responses (Labasi J M, P. N., Donovan C, McCurdy S, Lira P, Payette M M, Brissette W, Wicks J R, Audoly L, Gabel C A., Absence of the P2X7 receptor alters leukocyte function and attenuates an inflammatory response. J Immunol, 2002. 168(12)(Jun 15): p. 6436–45; Filippini, A., et al., Ecto-ATPase activity in cytolytic T-lymphocytes. Protection from the cytolytic effects of extracellular ATP. J Biol Chem, 1990. 265(1): p. 334–40). The present application discloses that RTF is the primary surface ATPase with this function.
RTF is the α-subunit of α2-isoform of vacuolar ATPase, and that RTF exists as a 70 kDa protein (Toyomura, T., et al., Three subunit a isoforms of mouse vacuolar H(+)-ATPase. Preferential expression of the a3 isoform during osteoclast differentiation. J Biol Chem, 2000. 275(12): p. 8760–5; Nichols, T. C., et al., Expression of a membrane form of the pregnancy-associated protein TJ6 on lymphocytes. Cell Immunol, 1994. 155(1): p. 219–29; Boomer, J. S., et al., Regeneration and tolerance factor's potential role in T-cell activation and apoptosis. Hum Immunol, 2000. 61(10): p. 959–71). A 20 kDa fragment can be cleaved, leaving the 50 kDa external membrane form (Nichols, T. C., et al., Expression of a membrane form of the pregnancy-associated protein TJ6 on lymphocytes. Cell Immunol, 1994. 155(1): p. 219–29). Current data support that RTF is known to have a role in certain forms of apoptosis (Boomer, J. S., et al., Regeneration and tolerance factor's potential role in T-cell activation and apoptosis. Hum Immunol, 2000. 61(10): p. 959–71; Boomer, J. S., et al., Regeneration and tolerance factor is expressed during T-lymphocyte activation and plays a role in apoptosis. Hum Immunol, 2001. 62(6): p. 577–88). It has also been shown equally that anti-RTF antibody can block RTF's ATPase activity, subsequently allowing ATP to bind P2Z and induce apoptosis. It has additionally been shown that RTF works in an antagonistic fashion versus the P2Z surface purinoceptor. U.S. Pat. No. 6,133,434 and International Patent Application (PCT) No. WO 95/33048 disclose that antibodies against P2Z receptors can be useful in treating a variety of diseases and conditions, including epilepsy, cognition, emesis, pain (especially migraine), asthma, peripheral vascular disease, hypertension, diseases of immune system, irritable bowel syndrome and premature ejaculation.
One possible mechanism for RTF to modulate inflammatory and immune responses is by RTF acting as an ATPase to reduce the level of extracellular ATP. ATP, released during injury or stress from tissues, infiltrating cells, and dying cells at the site of inflammation, interacts with the P2Z receptor. This interaction exacerbates the inflammatory response which leads to cell activation and the maturation and secretion of IL-1β. By controlling the degradation of extracellular ATP, RTF down regulates immune responses, including immune activation and inflammation. Thus, inhibiting the RTF activity leads to immune activation, which may lead to cell death, while enhancing the RTF activity leads to inhibition of inflammatory responses.
Any method that inhibits RTF activity can be employed in the present invention for immune activation. In a preferred embodiment, the method to inhibit RTF is by administering a RTF antagonist. The RTF antagonist can be a small molecule, a peptide, an antibody or a fragment thereof, and the like. The antibody can be either polyclonal or monoclonal. In one embodiment, the antagonist acts by binding to RTF to inhibit its activity. A preferred RTF antagonist is an anti-RTF antibody or a fragment thereof, and a preferred anti-RTF antibody is a monoclonal RTF antibody or a fragment thereof. A method to produce and purify a monoclonal RTF antibody is disclosed by Boomer et al. (Boomer, J. S., et al., Regeneration and tolerance factor's potential role in T-cell activation and apoptosis. Hum Immunol, 2000. 61(10): p. 959–71), which is incorporated herein by reference and made a part hereof. In another embodiment, the antagonist acts by inhibiting cellular expression of RTF. An example of such an antagonist includes, but is not limited to, an antisense nucleic acid which binds to the DNA coding for the RTF molecule. Using antisense nucleic acid to bind to DNA to inhibit cellular expression of proteins is well known in the art. Another example of antagonizing RTF is by inducing RNA interference (RNAi). The RNAi process induces the degradation of the target gene mRNA so as to silence the target gene expression. A typical RNAi process includes introducing into cells a double-stranded interfering RNA that comprises a sense RNA having the sequence homologous to the target gene mRNA and antisense RNA having the sequence complementary to the sense RNA. The double-stranded interfering RNA can be a small interfering double stranded RNA (also known as siRNA). The double-stranded interfering RNA can be introduced to the cells exogenously, or it can be expressed intracellular by incorporating into the cells an expression system to express the double-stranded interfering RNA. Intracellular expression is preferred for siRNA.
The RTF antagonist can be prepared as a pharmaceutical formulation by including one or more suitable or appropriate excipients. In an embodiment, the pharmaceutical formulation is a nanoparticle or a microparticle. The antagonist can be administered to the subject by any route including but not limited to parenteral, topical, nasal, pulmonary, ophthalmic, bucal, vaginal, transdermal, intrathecal, and oral
One of the results of inhibiting RTF activity is induction of cell apotosis, especially cancer cells, such as ovarian carcinoma cells. Thus, inhibiting RTF can be used as a method to treat cancer. Any of the methods described above which inhibit RTF can then be used as a method to treat cancer. An example of cancer that can be treated in the present invention is ovarian cancer.
Since inflammatory responses are the result of immune activation by the injured tissue, it is anticipated that enhancing RTF activity will result in inhibiting the inflammatory responses. Inflammation is known in many disorders which include, but are not limited to, arthritis (including but not limited to rheumatoid arthritis, spondyloarthopathies, gouty arthritis, osteoarthritis, systemic lupus erythematosus and juvenile arthritis), asthma, bronchitis, menstrual cramps, tendonitis, bursitis, and skin related conditions (such as psoriasis, eczema, burns and dermatitis), certain gastrointestinal conditions (such as inflammatory bowel disease, Crohn's disease, gastritis, irritable bowel syndrome and ulcerative colitis), vascular diseases, migraine headaches, periarteritis nodosa, thyroiditis, aplastic anemia, Hodgkin's disease, sclerodoma, rheumatic fever, type I diabetes, myasthenia gravis, multiple sclerosis, sarcoidosis, nephrotic syndrome, Behcet's syndrome, polymyositis, gingivitis, hypersensitivity, conjunctivitis, swelling occurring after injury, myocardial ischemia, certain central nervous system disorders (such as Alzheimer's disease and dementia), allergic rhinitis, respiratory distress syndrome, endotoxin shock syndrome, atherosclerosis, central nervous system damage resulting from stroke, ischemia, trauma, and the like. Many of the above inflammatory disorders are autoimmune disorders in which the body develops immune responses to its own protein. Thus, enhancing the activity of RTF can be used to treat or prevent inflammatory disorders, including autoimmune disorders, or their symptoms.
Any method that enhances the level of activity of RTF can be used to inhibit inflammatory responses and to treat or prevent inflammation in the present invention. In a preferred embodiment, the method is to administer to the subject an effective amount of RTF or a fragment thereof. In an embodiment, the RTF is an intracellular form which has a molecular weight of about 70 kDa. In another embodiment, the RTF is external membrane form having a molecule weight of about 50 kDa.
In one embodiment, the RTF can be isolated or purified from a mammalian source, such as murine or human, which includes but is not limited to, lymphocyte, macrophage, thymus, fetalplacental tissue, and the like. The lymphocyte can be a T-lymphocyte or a B-lymphocyte. The T- or B-lymphocyte preferably is activated.
In another embodiment, the RTF or a fragment thereof can be synthetic or a recombinant RTF, which can be derived, for example, from a nucleic acid sequence (e.g. cDNA) encoding the amino acid sequence of the RTF or the fragment. The nucleic acid sequence can be incorporated by recombinant techniques into an appropriate host organism for the expression of the RTF or the fragment. Examples of host organisms include, but are not limited to, bacteria, fungi, yeasts, protozoa, transgenic animals, transgenic plants, and the like. Recombinant techniques are well known to those skilled in the art and many biopharmaceuticals have been successfully produced by such techniques. A method for producing a recombinant RTF in E. coli is disclosed by Lee et al. (Lee, G. W., Bommer, J. S., Gilman-Sachs, A., Chedid A., Gudelj, L., Rukavina, D. and Beaman, K. D. Regeneration and tolerance factor of the human placenta induces IL-10 induction. Eur J Immunol, 2001. 31: p. 687–691) which is incorporated herein by reference and made a part hereof.
In a preferred embodiment of the present invention, the RTF or the fragment is formulated with one or more acceptable pharmaceutical excipients for administration to the subject. The RTF or the fragment can also be formulated as microparticles or nanoparticles. The microparticles or nanoparticles can further include ligands to deliver the microparticles or the nanoparticles to a target tissue such as the T- or B-lymphocyte or the macrophage. The RTF or the fragment can be administered to the subject by any acceptable route including, but not limited to, parenteral, topical, nasal, pulmonary, ophthalmic, bucal, vaginal, transdermal, intrathecal, oral and the like.
In another embodiment, the method to enhance RTF activity can be a method which enhances the expression of cellular RTF.
In yet another embodiment of the present invention, the method of treating inflammation by enhancing the RTF activity may include an additional step of administering to the subject a TNF-α antagonist. Since both IL-1β and TNF-α are known to cause inflammation, inhibiting the secretion of IL-1β by RTF and blocking the TNF-α activity by a TNF-α antagonist should have synergistic effects in treating inflammation. There are many known TNF-α antagonists. Examples include, but are not limited to, infliximab, etanercept, D2E7, CDP571, CDP870, thalidomide and its analogs, and phosphodiesterase type IV inhibitors.
J774A1 cells were maintained by allowing them to adhere to the bottom of a T75 flask with 25 mls of RPMI 1640 complete media at 37° C. in a 5% CO2 atmosphere. Cells were split into a new flask every 4 days using trypsin and a gentle wash with RPMI.
PBMC or J774A1 macrophages were suspended in 50 μl of RPMI at a density of 2.5×105 in a 96 well flat bottom plate and incubated with 10 μg of either 2C1 (anti-RTF) or an isotype matched control antibody for 45 mins at 37° C. in a 5% CO2 atmosphere. Cells were washed with PBS and re-suspended in 100 μl of assay buffer (5 mM KCl, 2 mM CaCl2, 2 mM MgCl2, and 1.5 μC of [γ-32P]ATP) in 1.5 ml eppendorf tubes. The ATPase reaction was allowed to continue for 10 mins at room temperature. 500 μl of 20% w/v activated charcoal (in distilled water) was added to scavenge any unused [γ-32P]ATP and allowed to sit for 10 mins on ice. The cells were centrifuged at 3200×g for 5 mins, pelleting the charcoal. 500 μl of supernatant containing released γ-32P was removed and added to scintillation vials with 3 mls of scintillation fluid and read in the scintillation counter for 1 min/tube (Filippini, A., et al., Ecto-ATPase activity in cytolytic T-lymphocytes. Protection from the cytolytic effects of extracellular ATP. J Biol Chem, 1990. 265(1): p. 334–40; Dombrowski, K. E., et al., Identification and partial characterization of an ectoATPase expressed by human natural killer cells. Biochemistry, 1993. 32(26): p. 6515–22; Dombrowski, K. E., et al., Antigen recognition by CTL is dependent upon ectoATPase activity. J Immunol, 1995. 154(12): p. 6227–37).
Approximately 2.5×105 PBMC were suspended in 100 μl of RPMI in a 96 well round bottom plate and a final concentration of either 3 mM ATP, 0.75 mM ATP, 10 μg anti-RTF, or 0.75 mM ATP+10 μg anti-RTF together was added. Cells were incubated in these conditions at 37° C. in 5% CO2 for 6 hours. Cells were washed twice in 0.01% BSA/PBS, and re-suspended in 100 μl binding buffer (10 mM HEPES pH 7.4, 140 mM NaCl, 2.5 mM CaCl2) with 5 μl of annexin-V/FITC (BD/Phanningen) for 15 mins. Cells were washed in binding buffer and re-suspended in 300 μl of binding buffer with 3 μl of 1 mg/ml propidium iodide. Apoptosis was measured by quantifying annexin-V binding by flow cytometry by gating on PI-/annexin-V+ cells (Vermes, I., et al., A novel assay for apoptosis. Flow cytometric detection of phosphatidylserine expression on early apoptotic cells using fluorescein labeled Annexin V. J Immunol Methods, 1995. 184(1): p.39–51).
A total of 2.5×105 cells were washed twice with 0.01% BSA/PBS for 5 mins and re-suspended in 100 μl of staining buffer. 5 μl of rabbit anti-P2X7 (P2Z) (Chemicon) antibody, 5 μl anti-RTF-FITC, or 5 μl of isotype matched control antibody was added to the appropriate tubes and allowed in react in the dark for 15 mins. Cell were washed again and re-suspended in 100 μl of staining buffer (1×PBS, 5% FBS) with 5 μl of anti-Rabbit biotinylated antibody (Pharmingen) and allowed to react for 15 mins. A third wash was performed and 2 μl of Streptavidin-PE (Pharmingen) was added for 15 mins. After a final wash, the cells were re-suspended in 300 μl of staining buffer and run on a BD Facscalibur flow cytometer.
J774 cells were suspended in 100 μl of RPMI in a 96 well round bottom plate at a density of 2.5×105 in on of the following conditions: 3 mM ATP, 0.75 mM ATP, 50 μg anti-RTF, or 0.75 mM ATP+10 μg anti-RTF. Cells were incubated at 37° C. in 5% CO2 for 30 mins in the presence of 1 μg PI or LY, washed in PBS, re-suspended in 300 μl PBS and analyzed in the BD Facscalibur flow cytometer.
For slides, J774 cells were grown in 4 well chamber slides for 2 days. The supernatant was removed and each chamber was incubated in one of the conditions described above for 15 mins in the presence of 1 μg PI or LY. The slides were washed in PBS, and incubated with 10μ Trypan blue for 5 mins, washed again and examined under a fluorescent microscope.
PBMC were obtained by ficoll separation and 2.5×105 cells per well were incubated in a 96 well plate in RPMI 1640 medium in the presence of 2 μg/ml PHA, or RPMI alone. After 72 hours both unstimulated, and stimulated cells were washed twice in PBS, permeabilized with ice cold 70% ethanol for 15 mins, and reacted with 7 μl anti-RTF-FITC, anti-CD8-PE (Pharmingen), or isotype control antibody for 15 mins. Cells were washed again, fixed with COULTER® fixative solution, and a cytospin was used to transfer them to a positively charged slide which was mounted with Dapco medium. Slides were then examined by confocal microscopy.
It has been previously shown that RTF expression in lymphocytes is dependent on activation (Boomer, J. S., et al., Regeneration and tolerance factor's potential role in T-cell activation and apoptosis. Hum Immunol, 2000. 61(10): p. 959–7). To characterize RTF expression in relation to P2Z expression during the immune response, the surface expression of RTF and P2Z on lymphocytes was measured following stimulation with PHA for 24–72 hours. In resting lymphocytes, RTF expression was 14.42±0.06% that of maximal expression while P2Z expression was 35.23±8.5%. RTF and P2Z expression increased together on the surface of the cells as stimulation time increased, with RTF and P2Z expression at 88.64±8.8% and 81.34±13.2% respectively at 72 hours (
The expression of RTF and P2Z on the J774A1 macrophage cell line has also been examined.
When lymphocytes examined by western blot at the time points stimulated above (
It is hypothesized that the 70 kDa form represents the intracellular form of RTF, while the 50 kDa form represents the external membrane form. To test this, the activated lymphocytes from
It is hypothesized that RTF regulates surface ATPase activity and anti-RTF blocks it. To demonstrate that RTF has surface ATPase activity, PBMC and J774A1 macrophages were incubated with either anti-RTF or isotype control antibody for 45 mins, and their surface ATPase activity was measured by [γ32-P]ATP degradation (Filippini, A., et al., Ecto-ATPase activity in cytolytic T-lymphocytes. Protection from the cytolytic effects of extracellular ATP. J Biol Chem, 1990. 265(1): p. 334–40; Dombrowski, K. E., et al., Identification and partial characterization of an ectoATPase expressed by human natural killer cells. Biochemistry, 1993. 32(26): p. 6515–22; Dombrowski, K. E., et al., Antigen recognition by CTL is dependent upon ectoATPase activity. J Immunol, 1995.154(12): p.6227–37). The PBMC incubated with anti-RTF had a 10 fold decrease in surface ATPase activity with 11,758±3,394 cpm compared to PBMC incubated with isotype antibody with a cpm of 115,592±23,891. (P<0.001;
Since RTF moves to the surface of the membrane as a 50 kDa size protein after stimulation in PBMC, and RTF regulates ATPase activity, it is desirable to demonstrate that RTF can prevent ATP induced apoptosis. For this purpose the macrophage cell line J774A1 is chosen. J774A1 cells were to be used as a model to demonstrate the interaction of RTF with P2Z because this cell line expresses both molecules constitutively and is known to undergo P2Z mediated, ATP induced apoptosis (Di Virgilio, F., The P2Z purinoceptor: an intriguing role in immunity, inflammation and cell death. Immunol Today, 1995. 16(11): p. 524–8; Coutinho-Silva, R. and P. M. Persechini, P2Z purinoceptor-associated pores induced by extracellular ATP in macrophages and J774 cells. Am J Physiol, 1997. 273(6 Pt 1): p. C1793–800). If the theory that RTF regulates surface ATPase activity and therefore regulates ATP binding to P2Z is correct, then it follows that anti-RTF and ATP would work together to generate more apoptosis than either alone by blocking the ATPase activity of RTF. When added together, at the same concentration as both alone, a near maximal amount of apoptosis occurred as measured by annexin-V (
A standard technique for detecting P2Z activity is used to demonstrate that the ultimate cause of the apoptosis inducing effect of RTF and ATP was due to P2Z activation (Di Virgilio, F., The P2Z purinoceptor: an intriguing role in immunity, inflammation and cell death. Immunol Today, 1995. 16(11): p. 524–8; Coutinho-Silva, R. and P. M. Persechini, P2Z purinoceptor-associated pores induced by extracellular ATP in macrophages and J774 cells. Am J Physiol, 1997. 273(6 Pt 1): p. C1793–800; Steinberg, T. H., et al., ATP4-permeabilizes the plasma membrane of mouse macrophages tofluorescent dyes. J Biol Chem, 1987. 262(18): p. 8884–8). When ATP interacts with P2Z, non-specific channels of about 0.9 kDa in size will open in the membrane (Dubyak, G. R. and C. el-Moatassim, Signal transduction via P2-purinergic receptors for extracellular ATP and other nucleotides. Am J Physiol, 1993. 265(3 Pt 1): p. C577–606; Di Virgilio, F., The P2Z purinoceptor: an intriguing role in immunity, inflammation and cell death. Immunol Today, 1995. 16(11): p. 524–8; Hickman, S. E., et al., P2Z adenosine triphosphate receptor activity in cultured human monocyte-derived macrophages. Blood, 1994. 84(8): p. 2452–6; Greenberg, S., et al., Extracellular nucleotides mediate Ca2+ fluxes in J774 macrophages by two distinct mechanisms. J Biol Chem, 1988. 263(21): p. 10337–43). This allows the testing for P2Z's influence by measuring the influx of molecules smaller than 0.9 kDa, to which the cell is normally not permeable. Propidium iodide (PI) (0.414 kDa) and lucifer yellow (LY) (0.46 kDa) should be allowed through if P2Z is activated, and trypan blue (TB) (0.96 kDa) should be excluded under all circumstances unless necrosis has occurred (Di Virgilio, F., The P2Z purinoceptor: an intriguing role in immunity, inflammation and cell death. Immunol Today, 1995. 16(11): p. 524–8; Coutinho-Silva, R. and P. M. Persechini, P2Z purinoceptor-associated pores induced by extracellular ATP in macrophages and J774 cells. Am J Physiol, 1997. 273(6 Pt 1): p. C1793–800; Steinberg, T. H., et al., ATP4-permeabilizes the plasma membrane of mouse macrophages tofluorescent dyes. J Biol Chem, 1987. 262(18): p. 8884–8). The same conditions used in the previous experiment were repeated to observe and measure the entry of propidium iodide or trypan blue in J774A1 cells. Thus P2Z influence would be characterized by cells that were PI and LY positive but TB negative.
Using flow cytometry, cells incubated with anti-RTF+0.75 mM ATP had pronounced channel formation judging from their incorporation of PI (
To show that RTF regulates IL-1β secretion, THP-1 macrophages were incubated with both 1 mM and 3 mM ATP, or anti-RTF and assayed for IL-1β secretion by ELISA. Since anti-RTF abrogates RTF function, our hypothesis was that anti-RTF would induce IL-β secretion, showing that RTF is a regulator for this molecule.
5×105 THP macrophage cells were stimulated with 5 ng/ml of LPS and 1×105 PBMC for 2.5 hours. These cells were then washed and incubated in a final concentration of either 0 ATP, 3 mM ATP, 1 mM ATP, or anti-RTF for a period of 3 hours. The supernatants were assayed for IL-1β by ELISA (R&D systems). pg IL-1β per well was calculated from the optical densities. Results are expressed as the mean of 3 independent experiments.
As shown in
A2780 ovarian carcinoma cells were grown in 96 well plates until 100% confluent. Wells were identified, and cells were then incubated with 3 mM ATP, 6 mM ATP, 20 μg of anti-RTF and 20 ug of anti-RTF combined with 3 mM ATP and 6 mM ATP. Cells were incubated for 18 hours at 37° C. in a 5% CO2 environment. Cells were then harvested and assayed using flow cytometry for Caspase 3 activation as an indicator for cell death. As shown in
Female athymic nude mice purchased from Harlan Sprague Dawley approximately 11 weeks old. All mice were injected with 200 μl of a 1:1 slurry of a Matrigel mix containing 5×106 A2780 ovarian carcinoma cells. Tumor cells were transplanted subcutaneously in the upper flank of the right leg. Two mice were untreated and kept as a control to measure tumor growth. The remaining six mice were injected with anti RTF antibody. All mice were left untreated for 1 week in order for a tumor and its vascular bed to become established. On the eighth day all mice that were treated were injected with 100 μg of anti RTF antibody in a volume of 100 μl of PBS. Injections were given in the tumor bearing flank of the animal. Antibody was not injected directly into the tumor, but was injected into the area of the tumor bed. Mice received 300 μg of antibody per week using a 28 gage needle. Mice were injected every Sunday, Tuesday and Friday. Injections took place over 5 weeks. The experiment was terminated when the control mice tumor burden became too obstructive for mice to ambulate.
The median tumor volume of the control animals after 5 weeks without anti-RTF treatment was 8448 mm3. The median tumor volume for the anti-RTF treated animals (n=6) was 364 mm3. In two of the treated animals no measurable tumor was observed (tumor volume range 0–1670). These results clearly indicate the possible usefulness of the antibody and or the inhibition of the RTF associated ATPase complex in tumor therapy
It should be understood that various changes and modifications to the presently preferred embodiments described herein will be apparent to those skilled in the art. Such changes and modifications can be made without departing from the spirit and scope of the present invention and without diminishing its intended advantages. It is therefore intended that such changes and modifications be covered by the appended claims.
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| Nov 15 2004 | BEAMAN, KENNETH | ROSALIND FRANKLIN UNIVERSITY OF MEDICINE & SCIENCE | ASSIGNMENT OF ASSIGNORS INTEREST SEE DOCUMENT FOR DETAILS | 015420 | /0527 |
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